Objective:Thisexperimentaimstodiscoveriftemperaturehasaneffectontheratesofseaurchinembryonicdevelopment.Byalteringtheexternalenvironment,theexperimentwilldetermineiftemperaturewillaffectthelengthofthefirstandsubsequentcellcyclesuptothepluteuslarvaestage. Introduction: SeaurchinembryosexhibitrADIalholoblasticcleavageinwhichthefirstandsecondcleavagesarebothmeridionalandperpendiculartoeachother.Thethirdcleavageisequatorial,andthefourthcleavagedividesunequallytoproducemesomeres,macromeres,andmicromeres(Gilbert,2003).Thesecleavagepatternsarewellunderstoodonagrouplevel,butitisnotcompletelyclearhowtheindividualcellsareregulatedonamolecularlevel.Onecanfollowtheeggfromfertilizationtoblastulatogastrulatopluteuslarvaeformation,butthisisusuallyperformedunderidealsituations.Iftheconditionschange,suchasthesaltconcentrationortemperatureofthewater,howwillthisaffectthedevelopmentoftheseaurchin? Manyprocesses,actinginsequenceorinparallel,makeupthecellcycle.ManystudieshaveshownhowthecellcycleisregulatedatthemolecularlevelinthecyclicaccumulationanddestructionofcyclinsandthecyclicactivityofMphase-promotingfactor(Meijeretal.,1991).However,onlysomeoftheseprocessesaffectthelengthofthecycle(Nurse,1990).Otherenvironmentalfactorshavebeensuggestedasadditionalregulatorsofthecellcycle.Forexample,temperaturehasbeenshowntohaveanumberofeffectsontheroleofvariousphasesofmitoticdivision,suchastherateofoxygenconsumptionandcarbondioxideproduction(Hoadley,1937).Researchershavefoundthatcellcycleeventsdiffergreatlyintheirdegreeoftemperaturedependence.Seaurchinsareoneorganismthatisaffectedbytemperature.Atemperature-dependentperiodexistsaftereggfertilizationinwhichthedurationofthecleavagecycleandnormaldevelopmentpatternsareaffectedbythetemperatureofthesurroundingenvironment(Yamada,K,andK.Mihashi,1998).SewellandYoung"sexperiment"TemperaturelimitstofertilizationandearlydevelopmentinthetropicalseaurchinEchinometralucunter"showedthateachseaurchinspecieshasanoptimalfertilizationtemperaturebasedontheaveragetemperaturefoundinitsnaturalhABItat(Sewell,M.A.andC.M.Young,1999).Thisoptimaltemperatureisnecessaryforthesuccessfuldevelopmentoftheembryosandpluteuslarvae(Katsuyuki,Y.,andK.Mihashi,1998).Anumberofspeciesofseaurchinsarefoundaroundtheworld.Eachspeciesthrivesintheirownuniqueenvironment.ThesubjectofthisexperimentisLytechinusvariegatus,whichisfoundintheGulfofMexicoandnormallydevelopsinwatertemperaturesnear22°C. Materials:maleandfemaleLytechinusvariegates100mLbeakerssterilesyringesandneedlespetridisheswithcoversartificialsaltwater(ASW)graduatedcylinderglassPasteurpipetsglassdepressionslidesicebucketaluminumfoil0.5MKCl14°Cincubator37°CincubatorThermometerlightmicrospcopedigitalcameraProcedure:1. 3. 4. 5. 6. 7. 8. 9. 10.When90%ormoreoftheeggshavecompletedcytokinesis,notethetimeafterfertilizationandtakestillphotographs. 11.Allowthefertilizedembryostodevelopfor24hours. 12.After24hours,transfer1dropofeachofthethreesamplesontodepressionslides. 13.Observethesampleunderthelightmicroscope.Takestillphotographsandcompareembryonicdevelopment. 14.48hoursafterfertilization,repeatsteps12and13. Results:Temperaturehadaneffectonthecleavageratesofdevelopingseaurchinembryos.Generally,thehighertheenvironmentaltemperature,thefastertheembryodivided.At37°C,theseaurchineggsreachedthefirstcellcleavageat40minutesafterfertilization,andcleavedthesecondtimeat65minutesafterfertilization.Abnormalitiesinthegastrulatingembryowereobservedat37°C.Underidealconditions,22°C,theembryosfirstcleavagecycleoccurredat60minutesafterfertilizationandthesecondcleavagecycleat100minutes.At14°C,thecleavageratewasdramaticallyslower,withthefirstdivisiontakingplaceat95minutesafterfertilization.Only50%oftheembryoscontinuedtodivide,inwhichtheyreachedthesecondcleavageat205minutesafterfertilization.Whenthecultureswerephotographed95minutesafterfertilization,theembryosincubatedat14°Chadonlydividedonce,thecontrolembryoshaddividedtwice,andtheembryosincubatedat37-38°Chadalreadydivided3times(Figure2). Twenty-fourhoursafterfertilization(Day2),thecontrolgrouphaddevelopednormally.Themajorityoftheembryosdisplayedarchenteronformationandweremotile.Notallembryoskeptat14°Chadhatchedbyday2.Theonesthathadhatcheddidnothavearchenteronsandwerenotmotile.Themajorityoftheembryoskeptat37°Chaddiedandlackedarchenterons.Theremainingembryoshaddevelopedabnormally,hadnothatchedandweresmallerthanthecontrolgroup(Figure3) Forty-eighthoursafterfertilization,allembryosofthecontrolgroupwereatthepluteuslarvaestage.At14°C,thevastmajorityoftheembryosweredeadandthosealivestilldidnotshowsignsofregulardevelopmentsuchasarchenteronformation.At37°C,thereweresomepluteuslarvaebutthemajorityoftheembryosweresmallandunhatched(Figure4). Discussion:Seaurchindevelopmentcanbealteredbyaseriesofenvironmentalchanges.Oneofthesechangesistemperature.Inourinitialexperiment,weshowedthatseaurchinsundergocleavagemorerapidlyinhighertemperatures.Inoursecondexperimentobservationswereextendedoveralongerperiodoftime.Weobservedthatchangesintemperaturecausedchangesindevelopment.Twenty-fourhoursafterfertilization,archenteronformationwasvisIBLeinthecontrolembryoswhereastheembryosintheothertwotemperatureswereundergoingabnormalandslowdevelopment.Lastly,48hoursafterfertilizationthecontrolembryowereallatthepluteuslarvaestagewhiletheotherembryoswereeitherdeadordevelopingabnormally.Overall,seaurchinembryodevelopmentistemperature-dependent,withtheprocessoccurringatafasterrateanddemonstratingabnormaldevelopmentsatwarmerthanidealtemperatures,andaslowerrate,andevencelldeath,takingplaceatcoolerthanoptimaltemperatures
Figure2.SeaUrchinembryos95minutesafterfertilization.Embryos(A.)incubatedat14°C,(B.)incubatedat22°C(Control),and(C.)incubatedat38°C.
Figure3.SeaUrchinembryos24hoursafterfertilization.Embryos(A.)incubatedat14°C,(B.)incubatedat22°C(Control),and(C.)incubatedat38°C.
Figure4.SeaUrchinembryos48hoursafterfertilization.Embryos(A.)incubatedat14°C,(B.)incubatedat22°C(Control),and(C.)incubatedat38°C.
